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基于蛋白质加合物测定的五氯苯酚肝结合研究。

Investigation of liver binding of pentachlorophenol based upon measurement of protein adducts.

出版信息

Biomarkers. 1996;1(4):232-43. doi: 10.3109/13547509609079363.

Abstract

Abstract Covalent binding of reactive metabolites of pentachloropheno (PCP) was investigated both in vitro andin vivo in the livers of male Sprague-Dawley rats via measurement of protein adducts. Cysteinyl adducts of quinones andsemiquinones in liver cytosolic (Cp) andnuclear (Np) proteins were assayed after catalytic cleavage by Raney nickel. Results from in vitro experiments confirmed that PCP metabolism produced tetrachlorobenzoquinones andthe comsponding tetrachlorobentosemiquinones which subsequently bound to sulphydryl groups in liver proteins. In vivo, the production of cysteinyl adducts increased with the administered dosage (0-40 mg PCP per kg body weight) andpresented evidence of saturable metabolism. Results suggest two metabolic pathways for PCP, including a high-affinity low-capacity pathway anda low-affinity high-capacity pathway. Time-course experiments in vivo andin vitro suggested that quinone adducts partlcipated in multiple substitution reactions with protein and/or non-protein thiols, andpointed to possible formation of protein-protein cross-links in vivo. The elimination rate constants of quinone adducts in vitro were about 0.35 h(-1) in liver Cp. The elimination of quinone adducts in vivo appeared to follow biphasic kinetics with rate constants for the terminal phase being 0.014 and0.008 h(-1) in liver Cp andNp, respectively.

摘要

摘要 本研究通过测定蛋白加合物,分别在雄性 Sprague-Dawley 大鼠的肝脏的体外和体内实验中,对五氯苯酚(PCP)的活性代谢产物的共价结合情况进行了研究。肝脏胞质(Cp)和核(Np)蛋白中的半胱氨酸加合物醌和半醌,经雷尼镍催化裂解后进行检测。体外实验结果证实,PCP 代谢产生四氯苯醌和相应的四氯苯半醌,随后与肝蛋白中的巯基结合。在体内,半胱氨酸加合物的生成随给药剂量(0-40mg PCP/kg 体重)增加而增加,呈现出可饱和的代谢特征。结果表明,PCP 有两种代谢途径,包括高亲和力低容量途径和低亲和力高容量途径。体内和体外的时间进程实验表明,醌类加合物部分参与了与蛋白和/或非蛋白巯基的多次取代反应,并指出体内可能形成了蛋白-蛋白交联。体外醌类加合物的消除速率常数约为 0.35h-1。体内醌类加合物的消除似乎呈现出双相动力学,终末相的速率常数分别为 0.014 和 0.008h-1,在肝脏 Cp 和 Np 中。

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